EXPRESSION AND PURIFICATION OF RECOMBINANT HUMAN BONE MORPHOGENETIC PROTEIN-7 IN Escherichia coli

Bone morphogenetic protein-7 (BMP-7) is a multifunctional cytokine of the transforming growth factor β superfamily, which induces bone formation and plays an important role during bone tissue repair and embryonic development. In this study, human BMP-7 (hBMP-7) cDNA was cloned and expressed in Escherichia coli, and its yield was approximately 30% of the total bacterial protein. After the bacteria were lysed by ultrasonication and repeated washing, inclusion bodies were extracted and dissolved using a high-strength denaturant. The monomer of rhBMP-7 was purified by ion-exchange chromatography, and the purity coefficient was approximately 96%. The protein was renatured with refolding buffers at different pH values. The renatured rhBMP-7 dimer protein in this study increased the alkaline phosphatase activity of NIH3T3 cells. This study may be helpful for the in vitro production and biomedical application of rhBMP-7 protein expressed in an E. coli expression system.     

细胞因子人MK基因的克隆及在大肠杆菌中的高效表达(简报)

细胞因子Midkine(简称MK)是新发现的一类肝素结合因子家族中的一员。1988年,Kadamatsu等利用差异杂交法在经维甲酸诱导分化的小鼠畸胎瘤细胞株HM-1中首先克隆到小鼠MK基因。人MK基因则最早是从λgt10人胚肾(20-24周)cDNA库和EMBL-3人胎盘基因组库获得。成熟     

蛛丝蛋白基因在大肠杆菌中表达研究

利用大腹园蛛基因组文库筛选获得一段693 bp基因片段,经分析该段基因处于鞭毛状丝基因重复区域,且其中包含了一个完整的重复框架。通过基因密码子优化,在其3′和5′端分别融合蛋白质亲和层析标签,克隆于pET30LIC表达载体中,在不同的大肠杆菌中进行表达试验。实验结果显示:经过密码子优化,融合目的蛋白基因在BL21(DE3)中得到了高效表达,产量达到25~30mg/L,纯化产物纯度达90%以上。SDS-PAGE和W estern-b lotting检测目的融合蛋白均与预期蛋白大小一致。     

HIV-1Gag蛋白在大肠杆菌和重组杆状病毒系统中的高效表达及通用型温控原核表达载体的构建

将中国株HIV－1B亚型的gag全基因序列,克隆到杆状病毒表达载体pfastbacI中,构建了重组质粒pfastGag,利用细菌／杆状病毒表达系统筛选重组杆状病毒,在昆虫细胞中高效表达了HIV－1Gag蛋白。通过改造原核表达载体pBV220和pET28,构建了一种新的通用型温控原核表达载体质粒pVV5,该载体携带PrPl串联温控启功子及His—Tag纯化标签,利于目的蛋白表达与纯化。将HIV－1gag基因的1148一1857编码序列,分别插入到pVV5b、pET28b的相应位点,构建了重组表达质粒pEG1b、pEG7b,二者在不同受体菌中,表达重组蛋白的量分别占全菌体蛋白总量的42％和28％。利用IMAC金属螯合层析柱,对包涵体中的重组p24蛋白进行纯化,纯度超过80％;纯化后的重组蛋白可与HIV－1型标准阳性血清发生较强的免疫学反应。     

密码子优化提高aiiaB546毕赤酵母表达活性

N-酰基高丝氨酸内酯酶是一类特异性降解N-酰基高丝氨酸内酯类信号分子(AHLs)的蛋白水解酶,通过水解AHLs生成酰基高丝氨酸,使AHLs失去活性,从而阻断病原菌的群体感应路径,使病原菌失去致病能力,其广泛存在于多种微生物中[1,2]。近年来N-酰基高丝氨酸内酯酶作为一种新型抗菌策略(群体感应淬灭策略)的工具酶而成为水产养殖防治细菌性疾病研究的热点[3—5]。     

人睫状神经营养因子的原核表达,纯化及其生物效应

人睫状神经营养因子（ｈＣＮＴＦ）克隆入ｐＢＶ２２０中，在ＤＨ５α菌株中表达，重组蛋白以包含体的形式存在，表达量为菌体总蛋白的５０％左右。经比较发现用２ｍｏｌ／Ｌ脲洗涤包含体可溶解大量可溶性细菌蛋白，且包含体损失较小。在高浓度变性剂条件下进行ｓｅｐｈａｒｃｙｌＳ－２００凝胶过滤，解决了纯化中ｈＣＮＴＦ易聚合的问题，在低浓度变性剂条件下进行ＤＥＡＥ离子交换，有利于蛋白活性的保持。经两步纯化后得到均一性ｈＣＮＴＦ，纯度达９５％以上。在自然状态下使ｈＣＮＴＦ复性。纯化复性后的ｈＣＮＴＦ对无血清培养的鸡胚背根节神经元和脊髓腹角运动神经元有明显的维持存活和促进生长发育的生物效应。     

甲型流感病毒核蛋白在大肠杆菌中的可溶性高效表达与纯化

为了在大肠杆菌中高效表达甲型流感病毒A/京科/30/95(H3N2)核蛋白NP,以便对原核表达的NP蛋白进行免疫原性研究,本研究通过密码子优化及全基因合成等方法,将3种形式的NP基因:与6×His标签融合的NP基因NP(His)、非融合的野生型NP基因NPwt及非融合的按大肠杆菌优势密码子改造的基因NP(O)分别插入原核表达载体pET-30a,构建了表达3种形式NP基因的3种原核表达质粒并研究不同质粒中NP蛋白的表达形式、条件、纯化工艺及抗原性。限制性酶切反应与测序表明,三种形式的NP基因均正确插入原核表达质粒pET-30a;SDS-PAGE凝胶电泳显示,三种形式的NP基因均能在大肠杆菌中表达,NP(O)基因的表达量最高;在不同温度诱导条件下,NP蛋白呈现可溶性表达,NP(O)基因可溶性高效表达的条件为:T=25℃,t=10 h;经阴离子交换和凝胶过滤层析两步纯化,可溶性表达的NP蛋白纯度可达90%;Western blot检测显示,纯化的NP能与流感病毒A/PR/8/34(H1N1)株感染小鼠的血清发生特异性结合。这些结果表明,非融合表达的密码子优化甲型流感病毒NP蛋白能在大肠杆菌中高效表达和纯化,同时保持良好的免疫反应活性。     

密码子优化的肺炎支原体P1蛋白在大肠杆菌中的克隆表达

目的:获得密码子优化的肺炎支原体P1黏附蛋白优势表位抗原基因,并在大肠杆菌中表达,为临床诊断试剂和疫苗研制打下基础。方法:采用生物信息学分析肺炎支原体P1蛋白的抗原表位,筛选特异性P1蛋白优势表位区;采用大肠杆菌优势密码子,设计上述P1蛋白优势表位基因序列;采用退火PCR技术合成上述基因,并利用载体pGEX-4T-2实现P1优势表位抗原在大肠杆菌中的表达;采用ELISA法对纯化的P1抗原活性进行测定。结果:肺炎支原体P1蛋白特异性抗原表位主要位于1154~1521 aa,获得的P1优化密码子基因平行突变37个稀有密码子和2个终止密码子;在大肠杆菌中表达的GST-P1融合蛋白的相对分子质量为65.9×103,纯化后重组抗原能与肺炎支原体感染者血清发生特异性的免疫反应。结论:采用密码子优化基因合成技术实现了肺炎支原体P1优势表位抗原在大肠杆菌中的高效表达,为肺炎支原体感染的诊断试剂研究提供了重要参考。     

人松弛素原样蛋白H2在大肠杆菌中的表达、分离纯化及鉴定

利用聚合酶链式反应方法 ,从含有人前松弛素原cDNA基因的质粒 pMALp2X-hRLXH2上得到人松弛素原H2的编码基因 ,亚克隆到温度诱导型原核表达载体pBV2 2 0上 ,转化大肠杆菌DH5α细胞。经 4 2℃温度诱导 ,获得了目的基因的高效表达。目的蛋白质以包含体的形式存在于大肠杆菌细胞中。菌体经过超声波破碎 ,包含体裂解 ,蛋白质的体外变性还原 ,复性 ,SephadexG 75凝胶过滤层析 ,反相快速蛋白质液相层析等一系列分离纯化过程 ,得到了高纯度的重组Met 人松弛素原样蛋白H2 ,得率约为 2～ 3mg/L。对纯化的目的蛋白质进行了SDS PAGE电泳纯度分析 ,氨基酸组成分析 ,通过基质辅助激光解吸电离飞行时间质谱法测得目的蛋白质的分子量为 183 90 .4 (理论计算值为 183 92 .3 )。     

AN OPTIMIZED PROTOCOL FOR OVERPRODUCTION OF RECOMBINANT PROTEIN EXPRESSION IN Escherichia coli

The gram-negative bacterium Escherichia coli (E. coli) offers a means for rapid, high-yield, and economical production of recombinant proteins. Here, a protocol for optimization of parameters involved in bacterial expression conditions is described. L-Asparaginase (ASNase II) was chosen as a model protein for our experiments. ASNase II gene (ansB) was cloned into the pAED4 plasmid and transformed into E. coli BL21pLysS (DE3)-competent cells. It was assumed that high cell density and high copy number of recombinant plasmid in the bacteria host could result in very high production of the recombinant protein. Circumstances for the overproduction of recombinant ASNase II including cell growth conditions, isopropyl β-D-1-thiogalactopyranoside (IPTG) level, ampicillin (Amp) concentration before and during IPTG induction, and cell density were optimized. Regarding the final optimization, overexpression of ASNase II was assessed on a large scale in LB medium. Periplasmic ASNase II was extracted using an alkaline lysis method. The extracted protein was purified by one-step DEAE-Sepharose fast-flow chromatography. ASNase II activity was considered an index for the protein expression. Applying the optimized practical protocol, protein production was significantly enhanced in comparison to the traditional IPTG induction method in the absence of a fermentor and can be applied for overexpression of other recombinant proteins.     

人胰岛素原基因在酵母中的分泌表达

 我们研究了外源基因——合成的人胰岛素原基因在酵母α因子系统中的表达和分泌。用表达载体YTI-15转化酵母63号株可得到每升约2毫克的人胰岛素原分泌产物。     

禁食促进下丘脑中摄食相关核团HAP1的表达

目的探讨下丘脑中的亨廷顿蛋白相关蛋白1（huntingtin-associated protein 1,HAP1）是否与摄食有关。方法免疫印迹法检测禁食对大鼠下丘脑HAP1表达的影响,RT-PCR法检测禁食对大鼠下丘脑HAP1 mRNA表达的影响,免疫组织化学染色法观察禁食对下丘脑与摄食调节有关核团内HAP1表达的影响。结果免疫印记分析和RT-PCR检测显示,与正常进食的大鼠比较,禁食1d、2d、3d、4d后大鼠下丘脑HAP1表达逐渐增多;免疫组织化学研究表明,弓状核、背内侧核、外侧下丘脑区内HAP1的表达在禁食后显著增多,而禁食对腹内侧核HAP1的表达无明显影响。结论下丘脑中的HAP1与摄食有关,可能参与了食欲的调节。     

大肠杆菌表达的重组人粒细胞-巨噬细胞集落刺激因子的纯化

对重组人粒细胞－巨噬细胞集落刺激因子（ｒｈＧＭ－ＣＳＦ）高效表达克隆ｐＺＷ．ＧＭ的表达产物进行了纯化,并对纯化的ＧＭ－ＣＳＦ进行了Ｎ端氨基酸序列分析。人ＧＭ－ＣＳＦ基因表达产物在大肠杆菌中以不溶性包涵体形式存在,经过超声破菌、包涵体抽提、凝胶过滤层析、复性、离子交换一系列化步骤,终产物纯度达９９％,按蛋白总量计算回收率达１０％,比活性达１×１０＾７ｕ／ｍｇ蛋白质。通过测定纯化人ＧＭ－ＣＳＦ的Ｎ端１     

STATISTICAL OPTIMIZATION OF GREEN FLUORESCENT PROTEIN PRODUCTION FROM Escherichia coli BL21(DE3)

An optimized cultivation condition is needed to maximize the functional green fluorescent protein (GFP) production. Six process variables (agitation rate, temperature, initial medium pH, concentration of inducer, time of induction, and inoculum density) were screened using the fractional factorial design. Three variables (agitation rate, temperature, and time of induction) exerted significant effects on functional GFP production in E. coli shake flask cultivation and were optimized subsequently using the Box–Behnken design. An agitation rate of 206 rpm at 31°C and induction of the protein expression when the cell density (OD_600nm) reaches 1.04 could enhance the yield of functional GFP production from 0.025 g/L to 0.241 g/L, which is about ninefold higher than the unoptimized conditions. Unoptimized cultivation conditions resulted in protein aggregation and hence reduced the quantity of functional GFP. The model and regression equation based on the shake flask cultivation could be applied to a 2-L bioreactor for maximum functional GFP production.     

表达重组人骨形态发生蛋白-7工程菌的发酵及表达产物的纯化

目的:研究表达重组人骨形态发生蛋白-7工程菌的发酵和表达产物的纯化工艺。方法:利用16L发酵罐发酵培养工程菌,设定了溶氧、搅拌速度、诱导时机、补料和培养基pH值等发酵条件;通过包涵体洗涤、离子交换层析法纯化目的蛋白。结果:工程菌目的蛋白质表达量占菌体总蛋白质的30%以上,纯化后目的蛋白的纯度可达98%。结论:建立了大肠杆菌高效表达人骨形态发生蛋白-7的发酵及纯化工艺。     

Functional activity of eukaryotic signal sequences in Escherichia coli: the ovalbumin family of serine protease inhibitors

It is widely assumed that the functional activity of signal sequences has been conserved throughout evolution, at least between Gram-negative bacteria and eukaryotes. The ovalbumin family of serine protease inhibitors (serpins) provides a unique tool to test this assumption, since individual members can be secreted (ovalbumin), cytosolic (leukocyte elastase inhibitor, LEI), or targeted to both compartments (plasminogen activator inhibitor 2, PAI-2). The facultative secretion of PAI-2 is mediated by a signal sequence proposed to be inefficient by design. We show here that the same internal domain that promotes an inefficient translocation of murine PAI-2 in mammalian cells is a weak signal sequence in Escherichia coli. In contrast, the ovalbumin signal sequence is much more efficient, whereas the corresponding sequence elements from LEI, maspin and PI-10 are entirely devoid of signal sequence activity in E.coli. Mutations that improve the activity of the PAI-2 signal sequence and that convert the N-terminal regions of maspin and PI-10 into efficient signal sequences have been characterized. Taken together, these results indicate that several structural features contribute to the weak activity of the PAI-2 signal sequence and provide new insights into the plasticity of the "hydrophobic core" of signal sequences. High-level expression of two chimeric proteins containing the PAI-2 signal sequence is toxic, and the reduced viability is accompanied by a rapid decrease in the membrane proton motive force, in ATP levels and in translation. In unc- cells, which lack the F0F1 ATP-synthase, the chimeric proteins retain their toxicity and their expression only affected the proton motive force. Thus, the properties of these toxic signal sequences offer a new tool to dissect the interactions of signal sequences with the protein export machinery.     

噬菌体T7溶菌酶及其融合蛋白在大肠杆菌中的表达

以噬菌体Ｔ７ＤＮＡ为模板,ＰＣＲ扩增Ｔ７溶菌酶基因,插入ｐＢｌｕｅｓｃｒｉｐｔＳＫ载体中,ＤＮＡ序列分析表明,克隆的Ｔ７溶菌酶基因和已报道的序列无氨基酸水平上的差异。将Ｔ７溶菌酶基因分别拼接在烟草病原相关蛋白（ＰＲ１ｂ）信号肽编码序列的３’末端和马铃薯卷叶病毒外壳蛋白（ＰＬＲＶＣＰ）基因靠近３’末端处,构建成两个融合蛋白基因。将Ｔ７溶菌酶及其融合蛋白基因插入大肠杆菌表达载体ｐＢＶ２２１,蛋白电泳及溶菌实验表明,Ｔ７溶菌酶基因在大肠杆菌中高效表达,其产物的表达量占菌体可溶性蛋白的２０％以上,ＰＬＲＶＣＰ的表达量并没有因Ｃ端融合Ｔ７溶菌酶而提高,高等植物的信号肽在大肠杆菌中也能起分泌信号作用。     

间隙连接蛋白Cx43在人胚肺和肺癌细胞表达的研究

细胞与细胞之间通过细胞膜上的间隙连接通道交换小分子和离子进行细胞间通讯,对细胞增殖分化调控和机体内环境稳定有重要作用。用间隙连接蛋白Ｃｘ４３ｃＤＮＡ探针Ｎｏｒｔｈｅｒｎ印迹杂交,Ｃｘ４３抗体免疫荧光染色和罗氏黄荧光染料传输方法检查,正常人胚肺细胞的Ｃｘ４３在ｍＲＮＡ和蛋白水平有高表达,Ｃｘ４３蛋白免疫荧光分布在间隙连接的部位,细胞间隙连接通讯功能明显。与正常相反,人肺癌ＰＧ系细胞Ｃｋ４３无论在ｍＲＮＡ或蛋白质水平都无表达,细胞通讯功能缺陷。结果表明Ｃｘ４３在培养的人胚肺细胞有功能性表达。人肺癌ＰＧ细胞通讯功能缺陷与Ｃｘ４３基因转录抑制有关。对Ｃｘ基因的抑癌基因性质进行讨论。     

Improved heterologous gene expression in Escherichia coli by optimization of the AT-content of codons immediately downstream of the initiation codon

Escherichia coli is the most frequently used host for heterologous gene expression. This study focuses on the effect of AT-rich codons immediately downstream of the initiation codon of the target gene. The third to sixth codons of ndx3, a Nudix hydrolase gene from Thermus thermophilus HB8, were engineered by introducing several silent mutations. As a result, the expression level of ndx3 increased in proportion to the AT-content in the third to sixth codons. This result suggests that incorporation of AT-rich codons can be utilized as a general strategy for improving the expression efficiency of a recombinant protein.